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可视化超螺旋 DNA 分子中的结构介导相互作用。

Visualizing structure-mediated interactions in supercoiled DNA molecules.

机构信息

Department of Physics, McGill University, Montreal, Quebec H3A 2T8, Canada.

Center for Cancer Research, National Cancer Institute, Bethesda, MD 20892, USA.

出版信息

Nucleic Acids Res. 2018 May 18;46(9):4622-4631. doi: 10.1093/nar/gky266.

Abstract

We directly visualize the topology-mediated interactions between an unwinding site on a supercoiled DNA plasmid and a specific probe molecule designed to bind to this site, as a function of DNA supercoiling and temperature. The visualization relies on containing the DNA molecules within an enclosed array of glass nanopits using the Convex Lens-induced Confinement (CLiC) imaging method. This method traps molecules within the focal plane while excluding signal from out-of-focus probes. Simultaneously, the molecules can freely diffuse within the nanopits, allowing for accurate measurements of exchange rates, unlike other methods which could introduce an artifactual bias in measurements of binding kinetics. We demonstrate that the plasmid's structure influences the binding of the fluorescent probes to the unwinding site through the presence, or lack, of other secondary structures. With this method, we observe an increase in the binding rate of the fluorescent probe to the unwinding site with increasing temperature and negative supercoiling. This increase in binding is consistent with the results of our numerical simulations of the probability of site-unwinding. The temperature dependence of the binding rate has allowed us to distinguish the effects of competing higher order DNA structures, such as Z-DNA, in modulating local site-unwinding, and therefore binding.

摘要

我们直接观察到超螺旋 DNA 质粒上的解旋部位与特定探针分子之间的拓扑介导相互作用,这是 DNA 超螺旋和温度的函数。可视化依赖于使用 Convex Lens-induced Confinement (CLiC) 成像方法将 DNA 分子包含在封闭的玻璃纳米孔阵列中。该方法在排除离焦探针信号的同时将分子困在焦平面内。同时,分子可以在纳米孔内自由扩散,允许准确测量交换率,与其他可能在结合动力学测量中引入人为偏差的方法不同。我们证明了质粒的结构通过其他二级结构的存在或不存在来影响荧光探针与解旋部位的结合。通过这种方法,我们观察到随着温度和负超螺旋的增加,荧光探针与解旋部位的结合速率增加。这种结合的增加与我们对解旋部位概率的数值模拟结果一致。结合速率的温度依赖性使我们能够区分竞争的更高阶 DNA 结构(如 Z-DNA)对局部解旋和因此的结合的调节作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fd52/5961182/a10e1693c858/gky266fig1.jpg

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